The Two Acetyl-coenzyme A Synthetases of Saccharomyces cerevisiae Differ with Respect to Kinetic Properties and Transcriptional Regulation

Berg, M. A.; Jong-Gubbels, Patricia de; Kortland, Christine J.; Dijken, Johannes P. van; Pronk, Jack T.; Steensma, H. Yde

doi:10.1074/jbc.271.46.28953

Cited by 216 publications

(194 citation statements)

References 28 publications

(22 reference statements)

Supporting

Mentioning

180

Contrasting

Order By: Relevance

“…The acetyl-CoA synthetase protein (Acs1p), showed an ϳ2.8-fold increase in protein abundance on the galactose carbon source, with no significant change in mRNA abundance. This finding is consistent with an earlier finding that suggests Acs1p is repressed by both glucose and ethanol (40).…”

Section: Discussionsupporting

confidence: 83%

Complementary Profiling of Gene Expression at the Transcriptome and Proteome Levels in Saccharomyces cerevisiae

Griffin¹,

Gygi²,

Ideker³

et al. 2002

Molecular & Cellular Proteomics

620

445

View full text Add to dashboard Cite

Using an integrated genomic and proteomic approach, we have investigated the effects of carbon source perturbation on steady-state gene expression in the yeast Saccharomyces cerevisiae growing on either galactose or ethanol. For many genes, significant differences between the abundance ratio of the messenger RNA transcript and the corresponding protein product were observed. Insights into the perturbative effects on genes involved in respiration, energy generation, and protein synthesis were obtained that would not have been apparent from measurements made at either the messenger RNA or protein level alone, illustrating the power of integrating different types of data obtained from the same sample for the comprehensive characterization of biological systems and processes. Molecular & Cellular Proteomics 1:323-333, 2002.The concept of discovery science, best illustrated by the human genome project (1, 2), involves the identification of the components of a system without the prior formulation of hypotheses as to how these components function (3). This scientific method has spawned what has become known as the "systems" approach to biology, which involves the comprehensive characterization of the components of a biological system (i.e. DNA, RNA, and proteins) as a whole, leading to insights into the responses of these components because of systematic perturbations to the system. The objective of the systems biology approach is to identify markers and mechanisms that are important to the function of the perturbed system, with the ultimate goal of developing computational models that enable the prediction of the response of the system to any given perturbation.Traditionally, studies measuring the effects of systematic perturbations have been carried out at the level of transcribed mRNA, most commonly using cDNA arrays and chip technologies (4 -7), or alternative methods for mRNA analysis such as serial analysis of gene expression (8), differential display (9), and cDNA fingerprinting (10). These technologies have been used to distinguish diagnostically between cell types (7,(11)(12)(13)(14)(15) and to differentiate between states (metabolic, activation, pathological) of a particular cell type (6, 16), as well as for the comprehensive analysis of cellular pathways and processes by targeted perturbations of cells (16 -19).Although the measurement of transcribed mRNA has proven to be very powerful in the discovery of molecular markers and the elucidation of functional mechanisms, alone it is not sufficient for the characterization of biological systems as a whole. This is based on several observations. First, comparison of absolute mRNA transcript abundances measured by serial analysis of gene expression (8) with the corresponding protein abundances expressed in exponentially growing Saccharomyces cerevisiae cells has shown that in many cases mRNA abundance is not a reliable indicator of corresponding protein abundance (20), and studies in other systems have reached similar conclusions (21, 22). Furthermore, attenuation...

show abstract

Section: Discussionsupporting

confidence: 83%

Complementary Profiling of Gene Expression at the Transcriptome and Proteome Levels in Saccharomyces cerevisiae

Griffin¹,

Gygi²,

Ideker³

et al. 2002

Molecular & Cellular Proteomics

620

445

View full text Add to dashboard Cite

show abstract

“…Strain and Growth Conditions-Wild-type Saccharomyces cerevisiae strain CEN.PK113-7D (MATa) (21) was grown at 30°C in 2-liter chemostats (Applikon, Schiedam, The Netherlands), with a working volume of 1.0 liter as described (22). Cultures were fed with a defined mineral medium that limited growth by glucose or ethanol with all other growth requirements in excess.…”

Section: Methodsmentioning

confidence: 99%

Comparative Proteome Analysis of Saccharomyces cerevisiae Grown in Chemostat Cultures Limited for Glucose or Ethanol

Kolkman

Olsthoorn

Heeremans

et al. 2005

Molecular & Cellular Proteomics

View full text Add to dashboard Cite

The use of chemostat culturing enables investigation of steady-state physiological characteristics and adaptations to nutrient-limited growth, while all other relevant growth conditions are kept constant. We examined and compared the proteomic response of wild-type Saccharomyces cerevisiae CEN.PK113-7D to growth in aerobic chemostat cultures limited for carbon sources being either glucose or ethanol. To obtain a global overview of changes in the proteome, we performed triplicate analyses using two-dimensional gel electrophoresis and identified proteins of interest using MS. Relative quantities of about 400 proteins were obtained and analyzed statistically to determine which protein steady-state expression levels changed significantly under glucose-or ethanollimited conditions. Interestingly, only enzymes involved in central carbon metabolism showed a significant change in steady-state expression, whereas expression was only detected in one of both carbon source-limiting conditions for 15 of these enzymes. Side effects that were previously reported for batch cultivation conditions, such as responses to continuous variation of specific growth rate, to carbon-catabolite repression, and to accumulation of toxic substrates, were not observed. Moreover, by comparing our proteome data with corresponding mRNA data, we were able to unravel which processes in the central carbon metabolism were regulated at the level of the proteome, and which processes at the level of transcriptome. Importantly, we show here that the combined approach of chemostat cultivation and comprehensive proteome analysis allowed us to study the primary effect of single limiting conditions on the yeast proteome. Molecular & Cellular Proteomics 4:1-11, 2005. Two-dimensional (2D)1 gel electrophoresis is a powerful tool to visualize hundreds of proteins at a time, which in combination with MS leads to their identification. This technology has been applied to the yeast Saccharomyces cerevisiae for the large-scale identification of more than 400 proteins, resulting in yeast reference maps (1-7). Other S. cerevisiae studies used 2D gel electrophoresis to obtain an overview of global changes in the yeast proteome as function of stimuli such as cadmium (8), lithium (9), H 2 O 2 (10), or sorbic acid (11).Most of these differential proteome studies on S. cerevisiae were performed on cells cultured in batch mode, i.e. in shake flasks or in reactors. Batch cultivation makes use of a closed system, in which all nutrients are in excess at the start of the cultivation. In terms of microbial physiology, such batch cultivation is relatively poorly controlled, because the composition of the growth medium and consequently the growth rate changes continuously. The yeast cells take up nutrients from the media while metabolites are excreted in the culture system, and their growth arrests when one of the nutrients is depleted or when too many toxic substrates are accumulated. The high concentration of carbon source in the culture, which is essential for this type of cultu...

show abstract

“…For chemostat cultivation, strains CEN.PK113-7D, Orange01 and Orange02 were grown at 30 • C in 2 litre chemostats (Applikon) with a working volume of 1.0 l, as described (van den Berg et al, 1996). Cultures were fed with a defined synthetic medium under glucose limitation (Climited) with all other growth requirements in excess and at a constant residual concentration.…”

Section: Strain Cultivationsmentioning

confidence: 99%

Heterologous carotenoid production in Saccharomyces cerevisiae induces the pleiotropic drug resistance stress response

Verwaal

Jiang

Wang

et al. 2010

Yeast

View full text Add to dashboard Cite

To obtain insight into the genome-wide transcriptional response of heterologous carotenoid production in Saccharomyces cerevisiae, the transcriptome of two different S. cerevisiae strains overexpressing carotenogenic genes from the yeast Xanthophyllomyces dendrorhous grown in carbon-limited chemostat cultures was analysed. The strains exhibited different absolute carotenoid levels as well as different intermediate profiles. These discrepancies were further sustained by the difference of the transcriptional response exhibited by the two strains. Transcriptome analysis of the strain producing high carotenoid levels resulted in specific induction of genes involved in pleiotropic drug resistance (PDR). These genes encode ABC-type and major facilitator transporters which are reported to be involved in secretion of toxic compounds out of cells. β-Carotene was found to be secreted when sunflower oil was added to the medium of S. cerevisiae cells producing high levels of carotenoids, which was not observed when added to X. dendrorhous cells. Deletion of pdr10, one of the induced ABC transporters, decreased the transformation efficiency of a plasmid containing carotenogenic genes. The few transformants that were obtained had decreased growth rates and lower carotenoid production levels compared to a pdr5 deletion and a reference strain transformed with the same genes. Our results suggest that production of high amounts of carotenoids in S. cerevisiae leads to membrane stress, in which Pdr10 might play an important role, and a cellular response to secrete carotenoids out of the cell.

show abstract

The Two Acetyl-coenzyme A Synthetases of Saccharomyces cerevisiae Differ with Respect to Kinetic Properties and Transcriptional Regulation

Cited by 216 publications

References 28 publications

Complementary Profiling of Gene Expression at the Transcriptome and Proteome Levels in Saccharomyces cerevisiae

Complementary Profiling of Gene Expression at the Transcriptome and Proteome Levels in Saccharomyces cerevisiae

Comparative Proteome Analysis of Saccharomyces cerevisiae Grown in Chemostat Cultures Limited for Glucose or Ethanol

Heterologous carotenoid production in Saccharomyces cerevisiae induces the pleiotropic drug resistance stress response

Contact Info

Product

Resources

About